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Previous Article | Next Article
The Journal of Neuroscience, January 1, 2001, 21(1):117-124
Expression of Brain-Derived Neurotrophic Factor in Cortical Neurons Is Regulated by Striatal Target Area
Josep M. Canals1, Núria Checa1, Sònia Marco1, Peter Åkerud2, Alice Michels1, Esther Pérez-Navarro1, Eduard Tolosa3, Ernest Arenas2, and Jordi Alberch1 1 Departament de Biologia Cel·lular i Anatomia Patològica, Facultat de Medicina, Universitat de Barcelona, Institut d'Investigacions Biomèdiques August Pi i Sunyer (IDIBAPS), Casanova 143, E-08036 Barcelona, Spain, 2 Laboratory of Molecular Neurobiology, Department of Medical Biochemistry and Biophysics, Karolinska Institute, Stockholm S-17177, Sweden, and 3 Servei de Neurologia, Hospital Clínic, Universitat de Barcelona, IDIBAPS, Villarroel 170, E-08036 Barcelona, Spain
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
Changes in BDNF expression after different types of brain insults are related to neuroprotection, stimulation of sprouting, and synaptic reorganization. In the cerebral cortex, an autocrine-paracrine mechanism for BDNF has been proposed because the distribution patterns of BDNF and TrkB expression are almost identical. Moreover, cortical BDNF is anterogradely transported to the striatum, suggesting a role of BDNF in the functional interaction between the two brain regions. Here we have examined the expression of this neurotrophin in the cerebral cortex after various striatal lesions. Intrastriatal injection of quinolinate, kainate, 3-nitropropionic acid, or colchicine increased BDNF mRNA levels in cerebral cortex. In contrast, stimulation of neuronal activity in the striatum did not change cortical BDNF expression. Both excitatory amino acids increased BDNF expression in neurons of cortical layers II/III, V, and VI that project to the striatum. Moreover, grafting a BDNF-secreting cell line prevented both the loss of striatal neurons and the cortical upregulation of BDNF induced by excitotoxins. Because retrograde transport in the corticostriatal pathway was intact after striatal lesions, our results suggest that striatal damage upregulates endogenous BDNF in corticostriatal neurons by a transneuronal mechanism, which may constitute a protective mechanism for striatal and/or cortical cells.
Key words: corticostriatal pathway; anterograde transport; excitatory amino acids; 3-nitropropionic acid; neurotrophins; synaptic activity; Huntington's disease
INTRODUCTION
Neurotrophins have been implicated in the regulation of development, neuronal survival, and adult synaptic plasticity (Thoenen, 1995
; Reichardt and Fariñas, 1997
Afferents from all areas of the cortex regulate neuronal activity in the striatal neurons via glutamate release. Excessive activation of glutamate receptors in the striatum produces selective degeneration of striatal projection neurons that resembles the pathological findings observed in Huntington's disease (Beal et al., 1986
Increase of cortical BDNF can also constitute an autocrine-paracrine trophic response for cortical neurons because BDNF protects cortical neurons from various types of insults (Shimohama et al., 1993
Our previous results showing that striatal excitotoxic lesions differentially regulated neurotrophin expression in various brain regions (Canals et al., 1998
MATERIALS AND METHODS
Animal injury. Male Sprague Dawley rats (140-210 gm) were anesthetized with pentobarbital (50 mg/kg, i.p.) and placed in a David Kopf Instruments (Tujunga, CA) stereotaxic apparatus (DK 900) with the incisor bar 5 mm above the interaural line. We used four to seven animals for each condition and time point studied. Quinolinate (QUIN) (34 or 68 nmol; Sigma, St. Louis, MO), kainate (KA) (2 or 6 nmol; Sigma), 3-nitropropionic acid (3-NPA) (500 nmol; Sigma), KCl (100 mM; Merck, Darmstadt, Germany), and PBS, pH 7.5, were injected in a volume of 1 µl into the left striatum at two coordinates [anteroposterior (AP), +2.3; lateral (L),
2.4 from bregma;
Some injections of QUIN, KA, or PBS to the striatum were performed from the contralateral hemisphere to avoid the effects of the needle-track injury in the ipsilateral cortex (AP,
In another set of experiments, glutamate antagonists were coinjected with 3-NPA at the following doses: kynurenic acid (Sigma), 60 nmol; dizocilpine maleate (MK801) (Tocris Cookson, Bristol, UK), 30 nmol; 6-cyano-7-nitroquinoxaline-2,3-dione disodium (CNQX) (Tocris Cookson), 1 nmol (n = 3 per group). Control rats were injected with the same doses of glutamate antagonists alone (n = 3 per group).
After lesioning, animals were housed separately with access to food and water ad libitum in a colony room maintained at a constant temperature (19-22°C) and humidity (40-50%) on a 12 hr light/dark cycle. All animal-related procedures were in accordance with the National Institute of Health Guide for the Care and Use of Laboratory Animals and approved by the local animal care committee of the Universitat de Barcelona (99/01) and by the Generalitat de Catalunya (99/1094).
Morphological analysis of the lesion size. Brains intrastriatally injected with QUIN, KA, 3-NPA, 3-NPA plus kynurenic acid, 3-NPA plus MK801, or 3-NPA plus CNQX were morphologically analyzed 3 d after lesion. The animals were deeply anesthetized in a CO2 chamber and transcardially perfused with 4% paraformaldehyde solution in 0.1 M sodium phosphate, pH 7.2. The brains were post-fixed 2 hr in the same solution, cryoprotected in 10% sucrose-PBS for 15 hr, and frozen in dry ice-cooled isopentane. Serial horizontal cryostat sections (14 µm) were processed for cresyl violet staining. Lesions were measured using Scion NIH Image on a computer attached to an Olympus Optical (Tokyo, Japan) microscope. Consecutive sections (26-29 sections per animal) were visualized, and the border of the lesion was outlined. The volume of the lesion was calculated by multiplying the sum of all the sectional areas (in square millimeters) by the distance between successive sections (0.2 mm) as described previously (Pérez-Navarro et al., 2000a
RNase protection assay. Rats were killed by decapitation at 2, 4, 6, 10, 16, or 24 hr after injury, brains were removed, and cerebral cortex was quickly dissected out, frozen on dry ice, and stored at
In situ hybridization studies. Animals were killed 6 hr after intrastriatal injection of PBS or excitatory amino acids (EAAs). Brains were dissected out and frozen in dry ice-cooled isopentane. Serial horizontal cryostat sections (14 µm) were processed for hybridization with radioactive BDNF riboprobe (Lindefors et al., 1995
-max x-ray film (Amersham Pharmacia Biotech) for 20 d and dipped in LM-1 photoemulsion (Amersham Pharmacia Biotech), exposed at 4°C for 2 months, developed with D19 (Eastman Kodak), fixed, and counterstained with cresyl violet staining. Some sections were processed for immunohistochemistry after the in situ hybridization. For this purpose, immediately after the last washes with SSC, the slides were coincubated with the primary antibodies GFAP (1:500; Dako A/S, Glostrup, Germany) and neuron-specific nuclear protein (NeuN) (1:100; Chemicon, Temecula, CA) overnight at 4°C. After three washes in PBS, the sections were coincubated with both secondary antibodies (anti-rabbit-FITC conjugated; 1:100; Vector Laboratories, Burlingame, CA; and anti-mouse-Texas Red conjugated; 1:100; Jackson ImmunoResearch, West Grove, PA), washed overnight in PBS, and dipped as mentioned above. Triple-labeling analysis was performed using a confocal microscope.
BDNF immunohistochemistry. Sections obtained with a cryostat (40 µm) were collected in PBS as free-floating sections and preincubated for 1 hr with PBS containing 10% methanol and 3% H2O2. Sections were then washed three times in PBS, permeabilized with 0.5% Triton X-100 (Sigma), and preincubated for 2 hr with 1.5% goat serum in PBS. After three washes in 0.1% Triton X-100 in PBS, tissue was incubated with the primary anti-BDNF antibody (1:200; Santa Cruz Biotechnology, Santa Cruz, CA) in PBS containing 0.1% Triton X-100 and 1.5% goat serum for 16 hr at 4°C. Sections were washed three times as above and incubated with a biotinylated goat anti-rabbit antibody (1:200; Vector Laboratories) for 1-2 hr at room temperature in the same buffer as the primary antibody. The immunohistochemical reaction was developed using the Vectastain ABC kit (Vector Laboratories) and intensified by incubation with 0.01% NiCl2.
Cell grafting of a BDNF-secreting cell line. Fischer 344 rat 3T3 fibroblasts transfected with BDNF (F3N-BDNF) (Neveu and Arenas, 1996
Studies of the corticostriatal transport. Studies of corticostriatal transport were performed by injecting a retrograde transport tracer (0.2 µl of Fluorogold; 2 mg/ml in PBS; Fluorochrome, Denver, CO) into the striatum in both hemispheres 3 d after unilateral QUIN or KA lesion (n = 3). The coordinates used for the tracer were the same as for the EAAs. Rats were transcardially perfused with 4% paraformaldehyde solution 48 hr after Fluorogold injection, and the brains were post-fixed and cryoprotected in 10% sucrose. Cryostat serial horizontal sections (25 µm) were mounted with immunofluore mounting medium (ICN, Costa Mesa, CA) and visualized under fluorescent microscope. All retrogradely labeled cells were counted in three separate regions (250 µm2/field): frontal, motor, and somatosensorial cortex. Retrograde signal was analyzed in 10-12 sections per animal separated by 175 µm. The number of positive cells on the side ipsilateral to the lesion was normalized to the number of cells on the contralateral side (nonlesioned).
To study the effect of blockage of axonal transport, a double injection of colchicine (2 × 1 µl at 20 µg/µl; Sigma) was performed 30 min before striatal excitotoxic injury. The coordinates used were the same as those described above for EAAs.
Statistical analysis. Results were normalized to the mean of sham-injected animals and expressed as a percentage of these data. Statistical analysis was performed using one-way ANOVA, followed by LSD (least significant difference t test) post hoc test.
RESULTS
Striatal excitotoxic injury increases BDNF mRNA levels in the ipsilateral cortex
Morphological analysis showed that intrastriatal injection of QUIN (68 nmol), KA (6 nmol), or 3-NPA (500 nmol) produced lesion sizes with the following volume rank order: KA (3.60 ± 0.10 mm3) > 3-NPA (3.23 ± 0.09 mm3) > QUIN (2.98 ± 0.08 mm3) (Fig. 1; see Fig. 6).
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Figure 1. Nissl-stained sections showing the striatal lesion (area inside dotted lines) induced by intrastriatal injection: A, C, QUIN (68 and 34 nmol, respectively); B, D, KA (6 and 2 nmol, respectively).
To examine BDNF expression in the cerebral cortex, after intrastriatal injection of QUIN or KA, we performed a sensitive RNase protection assay. Both glutamate receptor agonists increased BDNF mRNA in the cerebral cortex with a different profile (Fig. 2A). QUIN (68 nmol) induced a peak between 4 and 6 hr after lesion, reaching a maximum at 6 hr (306 ± 73%). The increase induced by KA occurred between 4 and 16 hr after injury, showing the highest levels of BDNF expression at 6 hr after injection (524 ± 115%).
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Figure 2. A, BDNF mRNA is upregulated in the cortex ipsilateral to excitotoxic lesion in the striatum. Intrastriatal QUIN injection (circles) induced a peak of expression between 4 and 6 hr. BDNF mRNA levels were also increased between 4 and 16 hr after KA-induced striatal injury (squares). Triangles represent sham-injected striata. Values are the mean ± SEM (n = 4-7; *p < 0.05; **p < 0.005). Autoradiograms show two representative experiments. B, Injection of QUIN or KA in the striatum through the contralateral cortex upregulated BDNF mRNA in the ipsilateral cortex. Values are mean ± SEM (n = 4; *p < 0.05).
To determine whether the regulation of cortical BDNF could be attributable to a local mechanical damage by the cannula, we performed intrastriatal injections from the contralateral hemisphere. In these conditions, BDNF mRNA was upregulated at 6 hr in the cortex ipsilateral to the intrastriatal QUIN or KA injection (270 ± 73 and 378 ± 87%, respectively) (Fig. 2B). No significant increase of BDNF expression was detected in the contralateral cortex.
In situ hybridization studies showed high levels of BDNF expression in the cortex ipsilateral to the lesioned striata (Fig. 3). At the two tested doses of QUIN (34 or 68 nmol) or KA (2 or 6 nmol), the upregulation of BDNF depended on the intensity of striatal damage (compare Figs. 1, 3). However, both NMDA and non-NMDA glutamate receptor agonists produced a similar pattern of expression in cortical layers II/III, V, and VI (Fig. 3D,E). This increase in BDNF mRNA levels was observed along the cerebral cortex, including the frontal, motor, and somatosensorial areas (Fig. 3B-E). No regulation of BDNF mRNA was observed in the hippocampus, indicating that the effects of QUIN or KA were specific to striatal neurons (Fig. 3B,C). Triple-labeling showed that BDNF mRNA was upregulated in cortical neurons (NeuN-positive cells) but not in glial cells (GFAP-positive cells) (Fig. 4A,B).
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Figure 3. In situ hybridization shows specific BDNF mRNA increased levels in the ipsilateral cortex after striatal EAA lesions. A, Autoradiograms showing a 20 d exposure of horizontal sections through brains receiving intrastriatal injection of PBS or high doses of EAAs (QUIN, 68 nmol; or KA, 6 nmol). B, C, Autoradiograms showing a 20 d exposure of intrastriatal injected brains with lower QUIN or KA doses (34 and 2 nmol, respectively). D, Bright-field photomicrographs of frontal, motor, and sensory cortical areas of QUIN-lesioned brains. E, Photomicrographs showing BDNF upregulation in the same cortical areas of KA intrastriatally injected animals. Scale bars, 150 µm.
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Figure 4. A, Photomicrographs showing triple-labeling of cortical layer II/III. NeuN-positive neurons are labeled in red, GFAP-positive astrocytes are labeled in green, and blue corresponds to the BDNF hybridization signal as assessed in radioactive in situ hybridization. B, High magnification of A. Note that GFAP-positive cells are negative for BDNF hybridization (open arrows), whereas NeuN-positive neurons are positive for BDNF mRNA signal (filled arrows). Some NeuN-positive neurons are negative for BDNF (arrowheads). Scale bars: A, 30 µm; B, 15 µm.
Immunohistochemical studies showed that the increase in BDNF protein coincided with the location of BDNF mRNA upregulation (Fig. 5). BDNF-positive cells were mainly located in layers II/III, V, and VI after intrastriatal QUIN or KA injury (Fig. 5B,C). The strongest BDNF immunolabeling was observed on cell bodies and apical dendrites of the pyramidal projecting neurons of layer V in the prefrontal cortex after QUIN or KA striatal injection (Fig. 5E,F).
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Figure 5. BDNF immunohistochemistry in the cerebral cortex reveals a pattern of expression similar to that observed for BDNF mRNA after striatal excitotoxic lesions. A, B, C, Immunolocalization of BDNF protein in the prefrontal cortex ipsilateral to PBS-, QUIN-, or KA-injected striata, respectively. D, E, F, Detailed photomicrographs of prefrontal layer V after injection of PBS, QUIN, or KA in the striatum, respectively. Scale bars: A-C, 200 µm; D-F, 100 µm.
Thus, our findings suggested that cortical BDNF is upregulated in response to either the loss of striatal cells or the increased neuronal activity by EAA. We therefore tested whether a striatal neurotoxin working on an energy-dependent mechanism could modify the cortical BDNF mRNA.
Cortical BDNF mRNA upregulation is specifically induced by striatal damage but not by increased neuronal activity
It has been shown that 3-NPA, an irreversible inhibitor of succinate dehydrogenase, produces selective loss of striatal projection neurons (Beal et al., 1993
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Figure 6. BDNF mRNA is transneuronally upregulated in the cortex by striatal cell death and not by synaptic activity per se. A-D, Nissl-stained sections in which unilateral lesions were performed. Note the areas of reduced staining (area inside dotted lines) in striata injected with the following: A, 3-NPA (500 nmol); B, 3-NPA (500 nmol) and kynurenic acid (Kyn; 60 nmol); C, 3-NPA (500 nmol) and an NMDA receptor antagonist (MK801; 30 nmol); and D, 3-NPA (500 nmol) and a non-NMDA receptor antagonist (CNQX; 1 nmol). E, Histogram represents BDNF mRNA levels from cerebral cortex 6 hr after intrastriatal injection of PBS, KCl, or 3-NPA alone or in combination with different glutamate receptor antagonists [kynurenic acid (Kyn), MK801, and CNQX]. Values, from three to four animals per condition, were normalized to those obtained in PBS-injected animals and are represented as mean ± SEM (*p < 0.05).
We also examined whether increased neuronal activity induced by KCl administration into the striatum modified BDNF mRNA expression in the cortex. Intrastriatal injection of 100 mM KCl did not affect cortical BDNF mRNA levels at 6 hr (104 ± 21%) (Fig. 6). Thus, combined, our observations suggested that cortical BDNF is upregulated after striatal damage. We therefore tested whether administration of neuroprotective factors for striatal neurons, such as BDNF, could prevent the cortical upregulation of BDNF expression.
The upregulation of BDNF mRNA in the cerebral cortex after striatal injury is prevented by intrastriatal administration of exogenous BDNF
We next examined whether administration of exogenous BDNF to the striatum modified the increase of cortical BDNF mRNA levels induced by intrastriatal EAA injections (Fig. 7). A BDNF-secreting cell line that protects striatal neurons against excitotoxicity (Pérez-Navarro et al., 1999
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Figure 7. Intrastriatal grafting of a BDNF-secreting cell line (F3N-BDNF) prevents the upregulation of BDNF mRNA in the cerebral cortex of EAA-lesioned animals. A, Values obtained from intrastriatal PBS injection in the F3A-MT-grafted striata were taken as 100%, and all other values were normalized to these data. Values are the mean ± SEM of four animals (***p < 0.001). B, Autoradiograms showing a 10 d exposure of brains hybridized with a BDNF 32P riboprobe in situ. Horizontal sections were obtained from animals intrastriatally grafted with the F3N-BDNF cell line and injected with PBS, QUIN, or KA. Although BDNF mRNA was detected in the cell line, no upregulation of cortical BDNF mRNA was observed.
Blockade of axonal transport does not prevent the BDNF upregulation in the cortex induced by striatal excitotoxic lesions
Intrastriatal injection of Fluorogold, a retrograde transport tracer, showed that the corticostriatal pathway was not affected by excitotoxic lesions in the target area (Fig. 8). The retrograde transport was studied in frontal, motor, and somatosensorial cortical areas (Fig. 8 A,B,C, respectively). No significant differences in cortical Fluorogold-labeled cells were observed after QUIN or KA intrastriatal lesion compared with the contralateral (nonlesioned) hemisphere.
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Figure 8. Excitotoxic striatal lesions do not affect the corticostriatal transport. Fluorogold-labeled cortical cells were counted in animals receiving bilateral injection of this retrograde tracer and unilateral injection of PBS, QUIN, or KA in the striatum. No differences between the three groups were observed. Number of labeled cells in the ipsilateral cortex to the lesioned striatum (I) were normalized to the number of Fluorogold-positive neurons from the contralateral hemisphere (nonlesioned; C). The values are represented as mean ± SEM of three animals per group.
To determine whether axonal transport is involved in the induction of BDNF mRNA expression in the cerebral cortex, colchicine was injected into the striatum. No retrograde transport of Fluorogold was observed in the cerebral cortex after intrastriatal colchicine administration, showing that retrograde transport was completely blocked (Fig. 9A, B). However, intrastriatal injection of colchicine alone or in combination with QUIN or KA upregulated BDNF expression similarly to EAA injection alone at 6 hr in the cortex (Fig. 9C). Thus, our results show that cortical neurons upregulate BDNF expression in the absence of either retrograde transport or in the absence of striatal neurons.
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Figure 9. BDNF mRNA is upregulated in the cerebral cortex 6 hr after disruption of corticostriatal transport. A, B, Photomicrographs comparing the retrograde transport of Fluorogold to the cortical layer V after injection of KA or colchicine, respectively. No labeling in the cerebral cortex was observed in colchicine-injected animals. Scale bars, 100 µm. C, Histogram represents cortical BDNF mRNA levels after intrastriatal injection of colchicine alone or in combination with QUIN or KA. Values are the mean ± SEM of four different animals for each condition, normalized to those obtained from PBS-injected animals (*p < 0.05).
DISCUSSION
Here we demonstrate that striatal damage or blockade of retrograde transport in corticostriatal neurons results in an upregulation of BDNF mRNA and protein in the cerebral cortex. Moreover, protection of the neostriatal neurons with exogenous BDNF prevented the upregulation of cortical BDNF induced by EAA. These results suggest that cortical BDNF upregulation may be an endogenous protective response to striatal damage.
Although QUIN and KA act through two different types of glutamate receptors, NMDA and non-NMDA, respectively, intrastriatal injection of either agonist at excitotoxic doses induced the same morphological pattern of cortical BDNF upregulation. The expression of BDNF was also increased in the cerebral cortex after intrastriatal injection of another neurotoxin, the 3-NPA (Beal et al., 1993
We next examined whether axonal communication is involved in the regulation of endogenous cortical BDNF mRNA levels. Intrastriatal injection of colchicine alone or in combination with QUIN or KA produced a large increase in cortical BDNF mRNA levels, reinforcing the idea that transneuronal BDNF expression is stimulated by the lack of the target area. These results suggest the existence of a constitutive factor released by striatal neurons that is retrogradely transported and regulates the cortical BDNF expression. In agreement with this hypothesis, it has been reported recently the existence of a neuron-restrictive silencer element that constitutively inhibits specific gene expression within the nervous system (Pathak et al., 1994
It has been shown previously that, after colchicine treatment, BDNF immunoreactivity is increased in cell bodies of cortical neurons, which send afferents to the striatum (Altar et al., 1997
Although our results are consistent with a long-distance effect of BDNF, we cannot rule out the possibility of a local action of BDNF in the cortex. Cortical BDNF upregulation could also constitute part of an autocrine-paracrine trophic response to protect cortical neurons from the loss of its target, the striatum. The study with Fluorogold also showed that retrograde transport is not affected in corticostriatal neurons by the lack of target neurons, raising the possibility of a potential role of BDNF in the maintenance of the cortical neurons. In fact, Giehl et al. (1998)
Analyses of neurotrophin expression in animal models of neurodegenerative diseases may help advance future understanding of the mechanism responsible for brain disease and development of neuroprotective treatments. We have shown previously that activation of glutamate receptors located on striatal neurons results in a specific pattern of neurotrophin expression during the development (Checa et al., 2000
In conclusion, our results show that striatal damage or blockade of retrograde transport in the corticostriatal pathway increases the levels of cortical BDNF, suggesting that this upregulation may constitute an adaptive mechanism against the progression of striatal and/or cortical neurodegeneration. Thus, stimulation of endogenous production of BDNF or administration of exogenous trophic factor may be a good therapeutic approach to prevent the progression of Huntington's disease.
FOOTNOTES Received July 31, 2000; revised Oct. 9, 2000; accepted Oct. 13, 2000.
This study was supported by Comisión Interministerial de Ciencia y Tecnología Grant SAF-99-0017 (Ministerio de Educación y Ciencia, Spain), Marató TV-3 Grant 97-TV1009, a grant from the Fundación Ramón Areces, a grant from the Swedish Medical Research Council (MFR), and BIOMED2 program of the European Commission Grant BMH4-CT96-0273. J.M.C. was supported by a short-term Human Frontiers Science Program fellowship. N.C. was supported by IDIBAPS, and S.M. was a fellow of CIRIT (Generalitat de Catalunya, Spain). We thank Dr. B. A. Sieber for critical reading of this manuscript, M. T. Muñoz and A. Nonell for technical assistance, and Anna Bosch and the Serveis Científico-Tècnics (Universitat de Barcelona) for support and advice in the use of confocal microscopy. We are also very grateful to Robin Rycroft for English language revision. This article is dedicated to the memory of Oriol Riba Canals, nephew of J.M.C.
Correspondence should be addressed to Dr. Jordi Alberch, Departament de Biologia Cel·lular i Anatomia Patològica, Facultat de Medicina, Universitat de Barcelona, Casanova 143, 08036 Barcelona, Spain. E-mail: alberch{at}medicina.ub.es.
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